A validated HPLC-MS/MS method for the simultaneous determination of ecdysteroid hormones in subminimal amounts of biological material.

IF 5 2区 医学 Q1 BIOCHEMISTRY & MOLECULAR BIOLOGY
Journal of Lipid Research Pub Date : 2024-10-01 Epub Date: 2024-09-05 DOI:10.1016/j.jlr.2024.100640
Lucie Marešová, Martin Moos, Stanislav Opekar, Michalina Kazek, Clemens Eichler, Petr Šimek
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引用次数: 0

Abstract

Ecdysteroids represent a large class of polyhydroxylated steroids which, due to their anabolic properties, are marketed as dietary supplements. Some ecdysteroids also act as important hormones in arthropods, where they regulate molting, development, and reproduction and many of these insects are miniature organisms that contain submicroliter levels of circulating biofluids. Analysis of ecdysteroids is further complicated by their very low abundance, large fluctuations during development, and difficult access to a pooled sample, which is important for quantitative measurements. In this work, we propose a new method that overcomes the described difficulties and allows validated quantification of four ecdysteroids in minimal amounts of biological material. After methanolic extraction, detectability of the ecdysteroids is increased 16- to 20-fold by conversion to their 14,15-anhydrooximes. These are further purified by pipette tip solid-phase extraction on a three-layer sorbent and subjected to HPLC-MS/MS analysis. Full validation was achieved using hemolymph from larvae of the firebug Pyrrhocoris apterus as a blank matrix and by the determination of ecdysteroids in a single Drosophila larva. The lower limit of quantifications for the four target ecdysteroids (20-hydroxyecdysone, ecdysone, makisterone A, and 2-deoxyecdysone) were 0.01; 0.1; 0.05; and 0.025 pg·ml-1 (20; 200; 100; 50 fmol ml-1), respectively, with very good accuracy, precision (expressed as relative standard deviation <15%) and recoveries (96%-119.9%). The application potential of the new method was demonstrated by quantification of ecdysteroids in various biological materials including human serum.

一种有效的 HPLC-MS/MS 方法,用于同时测定微量生物材料中的蜕皮激素。
蜕皮激素是一大类多羟基类固醇,由于具有同化特性,被作为膳食补充剂在市场上销售。一些蜕皮甾类化合物也是节肢动物体内的重要激素,它们能调节蜕皮、发育和繁殖,其中许多昆虫都是微型生物,它们体内的循环生物液体含量都在亚毫升以下。在这项工作中,我们提出了一种新方法,该方法克服了上述困难,可以在极少量的生物材料中对四种蜕皮激素进行有效定量。甲醇提取后,通过转化为 14、15-anhydrooximes,蜕皮激素的可检测性提高了 16-20 倍。这些物质通过三层吸附剂上的吸头固相萃取(PT-SPE)进一步纯化,并进行 HPLC-MS/MS 分析。使用萤火虫幼虫的血淋巴作为空白基质,并通过测定一只果蝇幼虫体内的蜕皮激素,对该方法进行了全面验证。四种目标蜕皮甾酮类化合物(20-羟基蜕皮甾酮、蜕皮甾酮、马基斯特酮 A 和 2-脱氧蜕皮甾酮)的 LLOQ 分别为 0.01;0.1;0.05;0.025 pg-mL-1(20;200;100;50 fmol-mL-1),准确度、精密度(RSD < 15%)和回收率(96% - 119.9%)都非常好。通过定量检测包括人血清在内的多种生物材料中的蜕皮激素,证明了新方法的普遍适用性。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
Journal of Lipid Research
Journal of Lipid Research 生物-生化与分子生物学
CiteScore
11.10
自引率
4.60%
发文量
146
审稿时长
41 days
期刊介绍: The Journal of Lipid Research (JLR) publishes original articles and reviews in the broadly defined area of biological lipids. We encourage the submission of manuscripts relating to lipids, including those addressing problems in biochemistry, molecular biology, structural biology, cell biology, genetics, molecular medicine, clinical medicine and metabolism. Major criteria for acceptance of articles are new insights into mechanisms of lipid function and metabolism and/or genes regulating lipid metabolism along with sound primary experimental data. Interpretation of the data is the authors’ responsibility, and speculation should be labeled as such. Manuscripts that provide new ways of purifying, identifying and quantifying lipids are invited for the Methods section of the Journal. JLR encourages contributions from investigators in all countries, but articles must be submitted in clear and concise English.
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